Presenting measurements of neuronal preparations with a novel CMOS-based microelectrode array at high-spatiotemporal-resolution on subcellular, cellular, and network level.
J. Müller, M. Ballini, P. Livi, Y. Chen, M. Radivojevic, A. Shadmani, V. Viswam, I. L. Jones, M. Fiscella, R. Diggelmann, A. Stettler, U. Frey, D. J. Bakkum, and A. Hierlemann, “High-resolution CMOS MEA platform to study neurons at subcellular, cellular, and network levels,” Lab Chip, vol. 15, no. 13, pp. 2767–2780, May 2015.
Reviewing the current understanding of microelectrode signals and the techniques for analyzing them, with focus on the ongoing advancements in microelectrode technology (in vivo and in vitro) and recent advanced microelectrode array measurement methods that facilitate the understanding of single neurons and network function.
M. E. J. Obien, K. Deligkaris, T. Bullmann, D. J. Bakkum, and U. Frey, “Revealing Neuronal Function through Microelectrode Array Recordings,” Front. Neurosci., 8:423, Jan 2015.
A high-resolution CMOS-based microelectrode array featuring 1,024 low-noise readout channels, 26,400 electrodes at a density of 3,265 electrodes per mm2, including on-chip 10bit ADCs and consuming only 75 mW.
M. Ballini, J. Muller, P. Livi, Y. Chen, U. Frey, A. Stettler, A. Shadmani, V. Viswam, I. L. Jones, D. Jackel, M. Radivojevic, M. K. Lewandowska, W. Gong, M. Fiscella, D. J. Bakkum, F. Heer, and A. Hierlemann, “A 1024-Channel CMOS Microelectrode Array With 26,400 Electrodes for Recording and Stimulation of Electrogenic Cells In Vitro,” IEEE Journal of Solid-State Circuits, vol. 49, no. 11, pp. 2705-2719, 2014.
Demonstrating a method to electrically visualize action potential propagation on axons and revealing
large variations in velocity.
D. J. Bakkum, U. Frey, M. Radivojevic, T. L. Russell, J. Muller, M. Fiscella, H. Takahashi, and A. Hierlemann, “Tracking axonal action potential propagation on a high-density microelectrode array across hundreds of sites,” Nature Communications, 4:2181, Jul 2013.
Recording and modeling extracellular action potentials of Purkinje cells at subcellular resolution.
U. Frey, U. Egert, F. Heer, S. Hafizovic, and A. Hierlemann, “Microelectronic System for High-Resolution Mapping of Extracellular Electric Fields Applied to Brain Slices,” Biosensors and Bioelectronics, vol. 24, no. 7, pp. 2191-2198, 2009.
Controlling BMP-2 expression to modulate the electrophysiological properties of cardiomyocytes using an HD-MEA for detailed monitoring.
C. D. Sanchez-Bustamante, U. Frey, J. M. Kelm, A. Hierlemann, and M. Fussenegger,
“Modulation of Cardiomyocyte Electrical Properties Using Regulated Bone Morphogenetic Protein-2 Expression,” Tissue Engineering Part A, vol. 14, no. 12, pp. 1969-1988, 2008.
@article{Kagan2021,
title = {In vitro neurons learn and exhibit sentience when embodied in a simulated game-world},
author = {Brett J. Kagan and Andy C. Kitchen and Nhi T. Tran and Bradyn J. Parker and Anjali Bhat and Ben Rollo and Adeel Razi and Karl J. Friston},
url = {https://www.biorxiv.org/content/10.1101/2021.12.02.471005v1 },
doi = {10.1101/2021.12.02.471005},
year = {2021},
date = {2021-12-03},
journal = {BioRxiv},
abstract = {Human brain organoids replicate much of the cellular diversity and developmental anatomy of the human brain. However, the physiological behavior of neuronal circuits within organoids remains relatively under-explored. With high-density CMOS microelectrode arrays (26,400 electrodes) and shank electrodes (960 electrodes), we probed broadband and three-dimensional extracellular field recordings generated by spontaneous activity of human brain organoids. These recordings simultaneously captured local field potentials (LFPs) and single-unit activity extracted through spike sorting. From spiking activity, we estimated a directed functional connectivity graph of synchronous neural network activity, which showed a large number of weak functional connections enmeshed within a network skeleton of significantly fewer strong connections. Treatment of the organoid with a benzodiazepine induced a reproducible signature response that shortened the inter-burst intervals, increased the uniformity of the firing pattern within each burst and decreased the population of weakly connected edges. Simultaneously examining the spontaneous LFPs and their phase alignment to spiking showed that spike bursts were coherent with theta oscillations in the LFPs. Our results demonstrate that human brain organoids have self-organized neuronal assemblies of sufficient size, cellular orientation, and functional connectivity to co-activate and generate field potentials from their collective transmembrane currents that phase-lock to spiking activity. These results point to the potential of brain organoids for the study of neuropsychiatric diseases, drug mechanisms, and the effects of external stimuli upon neuronal networks.},
keywords = {},
pubstate = {published},
tppubtype = {article}
}
Human brain organoids replicate much of the cellular diversity and developmental anatomy of the human brain. However, the physiological behavior of neuronal circuits within organoids remains relatively under-explored. With high-density CMOS microelectrode arrays (26,400 electrodes) and shank electrodes (960 electrodes), we probed broadband and three-dimensional extracellular field recordings generated by spontaneous activity of human brain organoids. These recordings simultaneously captured local field potentials (LFPs) and single-unit activity extracted through spike sorting. From spiking activity, we estimated a directed functional connectivity graph of synchronous neural network activity, which showed a large number of weak functional connections enmeshed within a network skeleton of significantly fewer strong connections. Treatment of the organoid with a benzodiazepine induced a reproducible signature response that shortened the inter-burst intervals, increased the uniformity of the firing pattern within each burst and decreased the population of weakly connected edges. Simultaneously examining the spontaneous LFPs and their phase alignment to spiking showed that spike bursts were coherent with theta oscillations in the LFPs. Our results demonstrate that human brain organoids have self-organized neuronal assemblies of sufficient size, cellular orientation, and functional connectivity to co-activate and generate field potentials from their collective transmembrane currents that phase-lock to spiking activity. These results point to the potential of brain organoids for the study of neuropsychiatric diseases, drug mechanisms, and the effects of external stimuli upon neuronal networks.
@inbook{Obien2019b,
title = {Large-Scale, High-Resolution Microelectrode Arrays for Interrogation of Neurons and Networks},
author = {Marie Engelene J Obien and Urs Frey},
url = {https://link.springer.com/book/10.1007%2F978-3-030-11135-9#about},
doi = {10.1007/978-3-030-11135-9},
year = {2019},
date = {2019-05-20},
publisher = {Springer},
abstract = {This book provides a comprehensive overview of the incredible advances achieved in the study of in vitro neuronal networks for use in basic and applied research. These cultures of dissociated neurons offer a perfect trade-off between complex experimental models and theoretical modeling approaches giving new opportunities for experimental design but also providing new challenges in data management and interpretation. Topics include culturing methodologies, neuroengineering techniques, stem cell derived neuronal networks, techniques for measuring network activity, and recent improvements in large-scale data analysis. The book ends with a series of case studies examining potential applications of these technologies.},
keywords = {},
pubstate = {published},
tppubtype = {inbook}
}
This book provides a comprehensive overview of the incredible advances achieved in the study of in vitro neuronal networks for use in basic and applied research. These cultures of dissociated neurons offer a perfect trade-off between complex experimental models and theoretical modeling approaches giving new opportunities for experimental design but also providing new challenges in data management and interpretation. Topics include culturing methodologies, neuroengineering techniques, stem cell derived neuronal networks, techniques for measuring network activity, and recent improvements in large-scale data analysis. The book ends with a series of case studies examining potential applications of these technologies.
@conference{Frey2017,
title = {Technology Trends and Commercialization of High-density Microelectrode Arrays for Advanced In-vitro Electrophysiology},
author = {Urs Frey and Marie Engelene J. Obien and Jan Muller and Andreas Hierlemann},
url = {https://ieeexplore.ieee.org/document/8050215/},
doi = {10.1109/ISCAS.2017.8050215},
issn = {2379-447X},
year = {2017},
date = {2017-05-28},
address = {Baltimore, MD, USA},
organization = {IEEE International Symposium on Circuits and Systems (ISCAS},
abstract = {Microelectrode arrays (MEAs) enable fast and high-throughput readout of cell's electrical signals. MEAs are currently used for phenotype characterization and drug toxicity/efficacy testing with iPSC-derived neurons and cardiomyocytes. A key advantage of MEAs is the capability to record and stimulate individual neurons at multiple sites simultaneously. We will present ongoing advancements of MEA technology, with a focus on achieving higher quality recordings by means of monolithic co-integration of circuitry on chip by using CMOS technology [1]. Such high-density MEAs with more than 3000 electrodes per mm2 are a suitable tool for capturing neuronal activity across various scales, including axons, somas, dendrites, entire neurons, and networks.},
keywords = {},
pubstate = {published},
tppubtype = {conference}
}
Microelectrode arrays (MEAs) enable fast and high-throughput readout of cell's electrical signals. MEAs are currently used for phenotype characterization and drug toxicity/efficacy testing with iPSC-derived neurons and cardiomyocytes. A key advantage of MEAs is the capability to record and stimulate individual neurons at multiple sites simultaneously. We will present ongoing advancements of MEA technology, with a focus on achieving higher quality recordings by means of monolithic co-integration of circuitry on chip by using CMOS technology [1]. Such high-density MEAs with more than 3000 electrodes per mm2 are a suitable tool for capturing neuronal activity across various scales, including axons, somas, dendrites, entire neurons, and networks.
@article{Kagan2021,
title = {In vitro neurons learn and exhibit sentience when embodied in a simulated game-world},
author = {Brett J. Kagan and Andy C. Kitchen and Nhi T. Tran and Bradyn J. Parker and Anjali Bhat and Ben Rollo and Adeel Razi and Karl J. Friston},
url = {https://www.biorxiv.org/content/10.1101/2021.12.02.471005v1 },
doi = {10.1101/2021.12.02.471005},
year = {2021},
date = {2021-12-03},
journal = {BioRxiv},
abstract = {Human brain organoids replicate much of the cellular diversity and developmental anatomy of the human brain. However, the physiological behavior of neuronal circuits within organoids remains relatively under-explored. With high-density CMOS microelectrode arrays (26,400 electrodes) and shank electrodes (960 electrodes), we probed broadband and three-dimensional extracellular field recordings generated by spontaneous activity of human brain organoids. These recordings simultaneously captured local field potentials (LFPs) and single-unit activity extracted through spike sorting. From spiking activity, we estimated a directed functional connectivity graph of synchronous neural network activity, which showed a large number of weak functional connections enmeshed within a network skeleton of significantly fewer strong connections. Treatment of the organoid with a benzodiazepine induced a reproducible signature response that shortened the inter-burst intervals, increased the uniformity of the firing pattern within each burst and decreased the population of weakly connected edges. Simultaneously examining the spontaneous LFPs and their phase alignment to spiking showed that spike bursts were coherent with theta oscillations in the LFPs. Our results demonstrate that human brain organoids have self-organized neuronal assemblies of sufficient size, cellular orientation, and functional connectivity to co-activate and generate field potentials from their collective transmembrane currents that phase-lock to spiking activity. These results point to the potential of brain organoids for the study of neuropsychiatric diseases, drug mechanisms, and the effects of external stimuli upon neuronal networks.},
keywords = {ETH-CMOS-MEA, In-Vitro, MaxOne},
pubstate = {published},
tppubtype = {article}
}
Human brain organoids replicate much of the cellular diversity and developmental anatomy of the human brain. However, the physiological behavior of neuronal circuits within organoids remains relatively under-explored. With high-density CMOS microelectrode arrays (26,400 electrodes) and shank electrodes (960 electrodes), we probed broadband and three-dimensional extracellular field recordings generated by spontaneous activity of human brain organoids. These recordings simultaneously captured local field potentials (LFPs) and single-unit activity extracted through spike sorting. From spiking activity, we estimated a directed functional connectivity graph of synchronous neural network activity, which showed a large number of weak functional connections enmeshed within a network skeleton of significantly fewer strong connections. Treatment of the organoid with a benzodiazepine induced a reproducible signature response that shortened the inter-burst intervals, increased the uniformity of the firing pattern within each burst and decreased the population of weakly connected edges. Simultaneously examining the spontaneous LFPs and their phase alignment to spiking showed that spike bursts were coherent with theta oscillations in the LFPs. Our results demonstrate that human brain organoids have self-organized neuronal assemblies of sufficient size, cellular orientation, and functional connectivity to co-activate and generate field potentials from their collective transmembrane currents that phase-lock to spiking activity. These results point to the potential of brain organoids for the study of neuropsychiatric diseases, drug mechanisms, and the effects of external stimuli upon neuronal networks.
@inbook{Obien2019b,
title = {Large-Scale, High-Resolution Microelectrode Arrays for Interrogation of Neurons and Networks},
author = {Marie Engelene J Obien and Urs Frey},
url = {https://link.springer.com/book/10.1007%2F978-3-030-11135-9#about},
doi = {10.1007/978-3-030-11135-9},
year = {2019},
date = {2019-05-20},
publisher = {Springer},
abstract = {This book provides a comprehensive overview of the incredible advances achieved in the study of in vitro neuronal networks for use in basic and applied research. These cultures of dissociated neurons offer a perfect trade-off between complex experimental models and theoretical modeling approaches giving new opportunities for experimental design but also providing new challenges in data management and interpretation. Topics include culturing methodologies, neuroengineering techniques, stem cell derived neuronal networks, techniques for measuring network activity, and recent improvements in large-scale data analysis. The book ends with a series of case studies examining potential applications of these technologies.},
keywords = {In-Vitro, Neuronal Networks},
pubstate = {published},
tppubtype = {inbook}
}
This book provides a comprehensive overview of the incredible advances achieved in the study of in vitro neuronal networks for use in basic and applied research. These cultures of dissociated neurons offer a perfect trade-off between complex experimental models and theoretical modeling approaches giving new opportunities for experimental design but also providing new challenges in data management and interpretation. Topics include culturing methodologies, neuroengineering techniques, stem cell derived neuronal networks, techniques for measuring network activity, and recent improvements in large-scale data analysis. The book ends with a series of case studies examining potential applications of these technologies.
@conference{Frey2017,
title = {Technology Trends and Commercialization of High-density Microelectrode Arrays for Advanced In-vitro Electrophysiology},
author = {Urs Frey and Marie Engelene J. Obien and Jan Muller and Andreas Hierlemann},
url = {https://ieeexplore.ieee.org/document/8050215/},
doi = {10.1109/ISCAS.2017.8050215},
issn = {2379-447X},
year = {2017},
date = {2017-05-28},
address = {Baltimore, MD, USA},
organization = {IEEE International Symposium on Circuits and Systems (ISCAS},
abstract = {Microelectrode arrays (MEAs) enable fast and high-throughput readout of cell's electrical signals. MEAs are currently used for phenotype characterization and drug toxicity/efficacy testing with iPSC-derived neurons and cardiomyocytes. A key advantage of MEAs is the capability to record and stimulate individual neurons at multiple sites simultaneously. We will present ongoing advancements of MEA technology, with a focus on achieving higher quality recordings by means of monolithic co-integration of circuitry on chip by using CMOS technology [1]. Such high-density MEAs with more than 3000 electrodes per mm2 are a suitable tool for capturing neuronal activity across various scales, including axons, somas, dendrites, entire neurons, and networks.},
keywords = {HD-MEA, In-Vitro},
pubstate = {published},
tppubtype = {conference}
}
Microelectrode arrays (MEAs) enable fast and high-throughput readout of cell's electrical signals. MEAs are currently used for phenotype characterization and drug toxicity/efficacy testing with iPSC-derived neurons and cardiomyocytes. A key advantage of MEAs is the capability to record and stimulate individual neurons at multiple sites simultaneously. We will present ongoing advancements of MEA technology, with a focus on achieving higher quality recordings by means of monolithic co-integration of circuitry on chip by using CMOS technology [1]. Such high-density MEAs with more than 3000 electrodes per mm2 are a suitable tool for capturing neuronal activity across various scales, including axons, somas, dendrites, entire neurons, and networks.
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